Nitrilase from arabis alpina, its encoding gene, vector, recombinant bacterial strain and uses thereof

ABSTRACT

The disclosure provides a nitrilase from  Arabis alpina , which belongs to genus  Arabis , family brassicaceae. The disclosure further provides the encoding gene, vector, recombinant bacterial strain, and the application in the manufacturing of (S)-3-cyano-5-methylhexanoic acid. The wet resting cells containing nitrilase Aa-Nit can kinetically resolve racemic IBSN at 1.2 M with a 42% conversion rate in 15 hr and &gt;99% ee value. The disclosure provides a regio- and stereoselective method for the preparation of (S)-3-cyano-5-methylhexanoic acid. This method provides an atom economical, mild, environmental friendly industrial method to manufacture (S)-3-cyano-5-methylhexanoic acid.

This application is a divisional application of U.S. patent application Ser. No. 15/246,626, filed Aug. 25, 2016, which claims the benefit of priority to Chinese Patent Application No. 201510535881.1, filed Aug. 27, 2015, the entirety of each are incorporated herein by reference.

Pursuant to 37 C.F.R. 1.821(c), a sequence listing is submitted herewith as an ASCII compliant text file named “CCHMP0002USD1_ST25.txt”, created on Aug. 24, 2017 and having a size of ˜5 kilobytes. The content of the aforementioned file is hereby incorporated by reference in its entirety.

1. TECHNICAL AREA

This invention relates to a method of manufacturing (S)-3-cyano-5-methylhexanoic acid. It further relates to a nitrilase from Arabis alpina and the application in the manufacturing of (S)-3-cyano-5-methylhexanoic acid.

2. BACKGROUND

Pregabalin (I, PGB), chemical name (S)-3-(aminomethyl)-5-methylhexanoic acid (I), is a 3-isobutyl substituted γ-aminobutanoic acid (Angew. Chem. Int. Ed. 2008, 47: 3500-3504). PGB is very effective in treating epilepsy, diabetic neuropathy pain, and post-herpetic neuralgia pain. It requires lower dosages and less frequent administration, has fewer side effects, lasts longer, and is well tolerated. PGB has become a blockbuster in global pharmaceutical markets.

(S)-3-Cyano-5-methylhexanoic acid (II) is a key chiral intermediate that can be converted to PGB through hydrogenation. Pfizer, Inc. has developed a second-generation, enzymatic process for PGB, where 2-carboxyethyl-3-cyano-5-methylhexanoic acid ethyl ester diethyl 2-(1-cyano-3-methylbutyl)malonate was resolved through Lipolase® catalysis, decarboxylated, and hydrolyzed under basic condition to afford II (Org. Process Res. Dev. 2008, 12: 392-398). This process requires decarboxylation and two hydrolysis steps, leading to low atom economy.

Nitrilase (EC 3.5.5.1) is an enzyme that can catalyze the hydrolysis of nitriles to ammonia and the corresponding carboxylic acid. Nitrilase has very strict regio- and stereo-selectivity and shows high potential in the manufacture of highly valuable active pharmaceutical ingredients. Pfizer's Xie reported that Arabidopsis thaliana nitrilase At-Nit1 could regio- and stereo-selectively convert racemic 2-isobutylsuccinonitrile (ISBN) into II (J. Mol. Catal. B: Enzym. 2006, 41:75-80). This process enjoys a very high atom economy. However, nitrilase At-Nit1 has low activity and only provides II with 17.5% yield when the substrate concentration was 150 mM (WO2005100580). Another enzyme NIT-102 could only provide II at 31.3% when the substrate was treated for 24 hr at 400 mM (WO2005100580). This method is difficult to industrialize because of the long reaction time and low substrate concentration. Thus, it is very necessary to find nitrilases with industrial potential for the manufacturing of II.

SUMMARY OF THE INVENTION

The goal of the current invention is to find a novel nitrilase that can regio- and stereoselectively convert ISBN into II. The nitrilase should show higher catalytic activity and better tolerance to substrate so that II could be manufactured in industrial scale. When at 400 mM, ISBN should be converted to II at least 42%.

An embodiment of the current invention is a nitrilase (Aa-Nit) from Arabis alpina, which belongs to family brassicaceae. The nitrilase's amino acid squence is shown in SEQ ID No. 1.

A further embodiment of the current invention covers any polypeptide segments or mutants obtained through knockout, insertion, replacement of one or more amino acid residues, as long as the sequence resembles 95% of SEQ ID No. 1.

Another embodiment of the current invention further covers a nitrilase's encoding gene. To realize the heterologous expression of soluble Aa-Nit in E. coli, the nucleotide (SEQ ID No. 2) corresponding to the amino acid sequence (SEQ ID No. 1) was synthesized through routine genetic engineering procedures.

Yet another embodiment of the current invention covers any nucleotide segments obtained through knockout, insertion, replacement of one or more nucleoside residues, as long as the sequence resembles 90% of SEQ ID No. 2.

Another embodiment of the current invention relates to a recombinant vector for the nitrilase encoding gene, and the recombinant genetically engineered bacterium obtained with the above-stated vector.

A further embodiment of the current invention relates to the method of preparing nitrilase Aa-Nit from the corresponding nitrilase gene. The nitrilase gene containing vector is introduced into the host cells to obtain the genetically engineered bacteria. The bacteria are cultured to obtain nitrilase-containing cells. The procedure is as follows: (1) Nitrilase Aa-Nit's nucleotide sequence was obtained through gene mining technique. (2) The synthesized nitrilase gene segment is inserted into pEt28b vector to afford the recombinant plasmid. (3) The recombinant plasmid is introduced into the host cell, preferably E. coli BL21 (DE3) to afford the corresponding engineered strain. (4) The engineered strain is inoculated into LB medium, grown to log phase, and induced with 0.1-0.2 mM IPTG at 28° C. for 12 hrs. (5) The cells are collected and the target protein size and expression is verified by SDS-PAGE electrophoresis (see FIG. 2).

Yet a further embodiment of the current invention relates to the application of nitrilase catalysis for the synthesis of II. Specifically, the engineered strain was fermented to obtain nitrilase-containing wet cells, which was used as the catalyst for the hydrolysis of racemic 2-isobutylsuccinimide in a pH 5.0-10.0 buffer (preferably in 100 mM, pH 8.0 Tris-HCl buffer) at 25-45° C. and stirred at 150 rpm (preferably at 30° C. and 150 rpm). After the hydrolysis is complete, II is isolated from the reaction mixture. The amount of catalyst used is 50 g/L of buffer based on the weight of the wet cells. The concentration of the substrate is 0.15-1.5 mol/L (preferably 0.7-1.2 mol/L).

The catalyst in the current invention is prepared as following: The nitrilase-containing engineered strain, preferably E. coli BL21 (DE3)/pET28b(+)-Aa-Nit, is inoculated into a liquid LB broth containing 50 μg/mL of kanamycin and grown for 12 hr at 37° C. The cultured broth was inoculated into a fresh liquid LB broth containing 50 μg/mL of kanamycin at 2% (v/v). The strain was grown at 37° C. until the cell concentration (OD₆₀₀) ca. 0.6 (0.4-0.8), and IPTG was then added to a final concentration of 0.2 mM to induce the protein expression 28° C. for 12 hr. After centrifugation at 4° C., 12000 rpm for 5 min, the wet cells are collected as catalyst.

A further embodiment of the current invention relates to the separation and purification method of II. After the reaction, the reaction mixture is centrifuged to remove E. coli. The supernatant is evaporated to ⅓ of the original volume. The temperature was maintained at 80° C. for 40 min to denature the proteins before the removal of the proteins through centrifugation. A preferred method of protein removal is through a further vacuum filtration. The filtrate is extracted with ethyl acetate (2× volume). The aqueous layer is acidified with 2 M HCl to pH 4.0. Extraction with ethyl acetate (2 volumes), followed by evaporation of ethyl acetate on rotavap, affords II as an oil.

The current invention provides a region- and stereo-selective enzyme for the manufacturing of II through hydrolysis of IBSN. The resting cells containing nitrilase Aa-Nit can kinetically resolve IBSN at 1.2 M with the conversion rate of 42% in 15 hr and ee>99%. The current invention provides an atom economical, mild, environmental friendly industrial method to manufacture II.

ILLUSTRATIONS

FIG. 1. Nitrilase Aa-Nit catalyzed kinetic resolution of IBSN.

FIG. 2. SDS-PAGE analysis of Nitrilase Aa-Nit. M: Molecular weight of proteins; 1: Induced expression of the target protein.

FIG. 3. Gas chromatography of nitrilase Aa-Nit catalyzed kinetic resolution of IBSN.

FIG. 4. Optimization of the pH of the reaction system.

FIG. 5. Optimization of the temperature of the reaction system.

EXAMPLES

The following examples are for the illustration of the current invention and in no way represents the scope of the current invention.

The main experimental materials were purchased from the following sources:

E. coli host strain: E. coli BL21 (DE3) Invitrogen Expression vector pEt-28b(+) Novagen Restriction endonucleases Xho I and Xba I Fermentas T4 DNA ligase TaKaRa Kanamycin TaKaRa IPTG Promega DNA marker and stain GoldView TaKaRa DNA gel extraction kit Axygen PCR Clean-up kit Axygen Plasmid extraction kit Axygen

Example 1—Preparation of Nitrilase Aa-Nit

(1) Nitrilase Aa-Nit amino acid sequence and nucleic acid sequence. A nitrilase amino acid sequence (Genbank No. KFK44999.1) was obtained via screening nitrilase gene sequence from protein database PDB and NCBI. The nitrilase comes from Arabis alpina, a plant belong to genus Arabis, family Brassicaceae. Based on the amino acid sequence of nitrilase, optimized codons from E. coli preferred codons, and the characteristics of vector pET28b(+), restriction enzyme cutting sites Xho I and Xba I were selected. The nitrilase-coding nucleic acid (shown in SEQ ID No. 2) and the coded amino acid sequence (shown in SEQ ID No. 1) were synthesized.

(2) Construction of recombinant strain. The nucleic acid segment was treated with restriction endonucleases Xho I and Xba I and recovered. The recovered gene and commercial vector pET28b(+) (pre-treated with restriction endonucleases Xho I and Xba I) were treated with T4 DNA ligase for 16 hr at 16° C. to give Intracellular recombinant expression vector pET28b(+)-Aa-Nit, which was introduced into E. coli BL21 (DE3) (Invitrogen), which was then spread onto a LB agar-plate containing 50 μg/ml of kanamycin and grown overnight at 37° C. The strains grown on the plate was randomly selected and the plasmid was extracted for agarose gel electrophoresis.

(3) Induced expression of nitrilase Aa-Nit. The recombinant genetically engineered E. coli BL21 (DE3)/pET28b(+)-Aa-Nit was inoculated into a liquid LB broth containing 50 μg/mL of kanamycin and grown for 12 hr at 37° C. The LB broth was inoculated into a fresh liquid LB broth containing 50 μg/mL of kanamycin at 2% (v/v). The strain was grown at 37° C. until the cell concentration (OD₆₀₀) reached 0.6 and IPTG was then added to a final concentration of 0.2 mM to induce the protein expression 28° C. for 12 hr and then centrifuged at 4° C. at 12000 rpm for 5 min. The wet cells are collected (resting cells, used for hydrolysis). The wet cells were washed with physiological saline twice, mixed well, and the cell solution was analyzed with SDS-PAGE electrophoresis. The results are shown in FIG. 2.

Example 2—Catalysis with Nitrilase Aa-Nit-Containing Resting Cells

The optimal pH, temperature, pH stability and substrate tolerance were investigated.

Reaction mixture (10 mL) was composed of buffer solution (10 mL, buffer), racemic IBSN (substrate), and wet resting cells (catalyst). The substrate's concentration was 0.4 mol/L. The catalyst quantity was 20 g of wet resting cells/L. The resting cells contained 70-90% of water. The reaction was initiated in a water bath shaker at 150 rpm for 0.5 hr and terminated with 2M HCl. The conversion rate was obtained with gas chromatography to ascertian the catalytic activity of the resting cells under various conditions.

(1) Determination of optimal pH. With the catalysis system defined above, the conversion rate of racemic IBSN was determined under various pH values (pH=5, 5.5, 6, 6.5, 7, 7.5, 8, 8.5, 9, 9.5, and 10) at 30° C. with substrate concentration at 0.4 mol/L and wet resting cells at 20 g/L. The buffers for various pH were acetic acid buffer (pH=5.0-6.0), sodium phosphate buffer (pH=6.0-7.2), Tris-HCl buffer (pH=7.0-9.0), and Gly-NaOH buffer (pH=9.0-10.0).

(2) Determination of optimal reaction temperature. With the catalysis system defined above, the reaction was carried out at various temperatures (25, 30, 35, 40, and 45° C.) in Tris-HCl buffer (100 mM, pH=8.0) with the substrate concentration at 0.4 mol/L and wet resting cells of 20 g/L. The conversion rate of racemic IBSN was determined.

(3) Determination of tolerance for maximal substrate concentration. With the catalysis system defined above, the reaction was carried out at various substrate concentrations (150 mM, 300 mM, 450 mM, 600 mM, 700 mM, 1 M, 1.2 M, and 1.5 M) in 10 mL of Tris-HCl buffer (100 mM, pH=8.0) with wet resting cells of 20 g/L. The conversion rate of racemic IBSN was determined.

The results show that nitrilase Aa-Nit-containing resting cells exhibit highest catalytic activity at pH 8.0, and the optimal reaction temperature is 30° C. The maximal substrate concentration tolerated is 1.2 M.

Example 3—Application of Nitrilase Aa-Nit-Containing Resting Cells

Kinetic resolution of racemic IBSN. The reaction is shown in FIG. 1. To a Tris-HCl buffer (10 mL, 100 mM, pH 8.0) was added racemic IBSN to reach 1.2 M, and 0.5 g of wet resting cells prepared in Example 1. The mixture was shaken at 30° C. for 15 hr in a water bath shaker. A 500 μL sample was taken every 3 hr and the reaction was quenched with 200 μL of 2 M HCl. The mixture was extracted with 800 μL of ethyl acetate, shaken, and centrifuged (12000×g, 2 min). The supernatant was dried with anhydrous sodium sulfate and analyzed with gas chromatography.

(1) Determination of conversion rate and ee value with chiral gas chromatography. The amount of substrate and product present in the extract was determined with chiral gas chromatography (GC-14 C, Shimadzu, Japan). The capillary tube was BGB-174 (BGB Analytik, Switzerland). Gas chromatography conditions are below:

Sample amount 1 μL Inlet and detector temperature 220° C. Column temperature 160° C. Carrier gas Helium Flow rate 1.6 mL/min Split ratio 30:1 The conversion rate and ee value were calculated according to literature method reported by Rakels et al. (Enzyme Microb Technol, 1993, 15: 1051).

(2) Isolation and purification of II. After the reaction, the reaction mixture is centrifuged to remove E. coli. The supernatant is evaporated to ⅓ of the original volume. The temperature was maintained at 80° C. for 40 min to denature the proteins before the removal of the denatured proteins through centrifugation. The supernatant was vacuum filtered to remove more proteins. The filtrate was extracted with ethyl acetate (2× volume). The aqueous layer is acidified with 2 M HCl to pH 4.0. Extraction with ethyl acetate (2× volume), followed by evaporation of ethyl acetate on rotavap, affords II as an oil (ee>99.5%).

The results show that the resting cells containing nitrilase Aa-Nit can kinetically resolve IBSN at 1.2 M with the conversion rate at 42% in 15 hr and ee_(p)>99%. Thus, nitrilase Aa-Nit catalysis disclosed in the current invention provides a mild method to manufacture II with high conversion rate and optical purity.

It is understood that the working examples are only for illustration so that those skilled in the art would understand the current invention and be able to reduce the current invention to practice. These examples are in no way to limit the scope and extent of the current invention. Any equivalent modifications or changes based on the current invention should be covered by the current invention.

REFERENCES CITED

-   Enzyme Microb Technol, 1993, 15: 1051 -   Org. Process Res. Dev. 2008, 12: 392-398 -   Angew. Chem. Int. Ed. 2008, 47: 3500-3504 -   J. Mol. Catal. B: Enzym. 2006, 41: 75-80 -   WO2005100580 

1. (canceled)
 2. A nitrilase encoding gene comprising the nucleoside sequence shown in SEQ ID No.
 2. 3. A recombinant vector comprising the nitrilase encoding gene of claim
 2. 4. A recombinant bacterial strain comprising the recombinant vector of claim
 3. 5-8. (canceled) 